A dual-functional module cellular electrochemical sensing platform for simultaneous detection guanine and xanthine

黄嘌呤 重复性 检出限 再现性 电化学电池 生物系统 化学 电化学 鸟嘌呤 活力测定 分析化学(期刊) 材料科学 色谱法 细胞 纳米技术 电极 生物化学 生物 物理化学 核苷酸 基因
作者
Shumeng Zhang,Jiwen Cui,Shi Zhou,Yanli Zhao,Jinlian Li,Dongmei Wu
出处
期刊:Biosensors and Bioelectronics [Elsevier BV]
卷期号:226: 115104-115104 被引量:8
标识
DOI:10.1016/j.bios.2023.115104
摘要

The separation of the superimposed electrochemical signals of intracellular guanine (G) and xanthine (X) is difficult, which is great obstacle to the application of cell electrochemistry. In this paper, independent functional modules, G-functional module (G-FM) and X-functional module (X-FM), were constructed by molecular imprinting technology for sensitive detection of G and X without mutual interference, then integrated in dual-functional module cellular electrochemical sensing platform (DMCEP) as signal sensing units. DMCEP transmitted signals of G and X in cells synchronously to two windows by two signal sensing channels, and achieved the separation of superimposed signals of G and X in cells. DMCEP exhibited satisfactory reproducibility with relative standard deviation (RSD) of 3.10 and 2.22 %, repeatability with RSD of 3.72 and 3.05 % for G and X detection, and detection limit 0.05 μΜ for G and 0.06 μΜ for X. Good linear relationships between cell concentrations and the signals of G and X on DMCEP were shown in range of 0.75–85 × 106 and 3–85 × 106 cells/mL, respectively. The growth of MCF-7 cells was tracked by DMCEP, and showed consistent trend with the cell counting method, while the change of cell viability from lag to logarithmic phase captured by DMCEP was earlier than that of cell counting method. This strategy provided the foundation for the establishment of the cell viability electrochemical detection method, and new insights into the simultaneous recording of other analyses with superimposed peak positions and the simultaneous tracking of multiple biomarkers.
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